Testing on
Bacteria
5.1.5 Student Resource Sheet
Introduction
Biochemical tests are the most definitive way to identify
bacterial species. Each biochemical test helps determine a
property or characteristic specific to a certain bacterial species.
These tests determine which growth media the bacteria will
grow on and identify the end products of their metabolic
processes, such as the wastes they excrete. For example, in one
biochemical test, the bacterial sample is inoculated in a growth
media containing a specific nutrient that only certain bacterial
samples are able to metabolize, or break down. The media also
contains an indicator. If the bacterial sample metabolizes the
nutrient, it excretes acid as a waste product, causing the
indicator to change color, indicating a positive result. Many
tests often need to be performed in order to positively identify a
bacterium. Laboratories have developed shortcuts that allow
scientists to perform several biochemical tests at one time. The
following slides contain a description of each of the biochemical
tests performed on Annas bacterial sample.
Arabinose Test
Test to determine if the microbe can ferment
the sugar arabinose as a food source. The
microbe is incubated in
phenol red arabinose broth for 24 hours. If the
microbe ferments arabinose, the media
become acidic, causing a color change from
red to yellow.
Catalase Test
Test to identify organisms that produce the
enzyme catalase. This enzyme detoxifies
hydrogen peroxide by breaking it down into water
and oxygen gas. The bubbles resulting from
production of oxygen gas clearly indicate a
catalase positive result.
Gelatin Hydrolysis
Testto determine if the microbe can use the
protein gelatin as a source of carbon and
energy for growth. The microbe is incubated
in nutrient gelatin. If the microbe uses
gelatin, the medium changes from semisolid
to liquid and cannot be resolidified.
Glucose Fermentation
Test
Test to determine if the microbe
can ferment the sugar glucose.
The microbe is grown in a broth
that contains glucose and the
pH indicator, phenol red. If an
organism is capable of
fermenting the sugar glucose,
then acidic byproducts are
formed and the pH indicator
turns yellow.
H2S
Indole Test
Test to determine if the microbe produces indole
as a byproduct from the metabolism of the amino
acid tryptophan. Ifindoleis produced, it will react
with a chemical reagent added after incubation to
produce a color change. There are two media that
are used for this test:Sulfide-Indole-Motility (SIM)
mediumandTryptone brothmedium.In SIM
media, indole reacts with added Kovacs reagent
to form rosindole dye which is red in color
Lactose Fermentation
Test
Test to determine if the microbe can ferment
the sugar lactose as a food source. The
microbe is incubated in
phenol red lactose broth for 24 hours. If the
microbe ferments lactose, the media become
acidic, causing a color change from red to
yellow
Lysine Decarboxylase
Test
Test to determine if the microbe can use the
amino acid lysine as a food source. The microbe is
incubated in lysine decarboxylase broth. The
microbe must first use the glucose present to
cause the pHto drop, which causes the color to
change from purple to yellow. Once the medium
has been acidified, the enzyme lysine
decarboxylaseis activated. The culture is
incubatedan additional 24 hoursat 35-37C to
allow the microbe to now use thelysine. The final
results are then observed at 48 hours. Change
back to purple from yellow indicates a positive
test for lysine decarboxylase. Failure to turn
yellow at 24 hours or to revert back to purple at
48 hours indicates a negative result.
Motility Test
Test to determine whether an organism is
equipped with flagella and thus capable of
swimming away from a stab mark. If the entire
tube is turbid, or cloudy, this indicates that the
bacteria have moved away from the stab mark
and are motile. If the stab mark is clearly visible
and the tube is not turbid, the organism is likely
non-motile.
Ornithine
Decarboxylase Test
Test to determine if the microbe can use the
amino acid ornithine as a food source. The
microbe is incubated in ornithine decarboxylase
broth. The microbe must first use the glucose
present to cause the pHto drop, which causes the
color to change from purple to yellow. Once the
medium has been acidified, the enzyme ornithine
decarboxylaseis activated. The culture is
incubatedan additional 24 hoursat 35-37C to
allow the microbe to now use theornithine. The
final results are then observed at 48 hours.
Change back to purple from yellow indicates a
positive test for ornithine decarboxylase. Failure
to turn yellow at 24 hours or to revert back to
purple at 48 hours indicates a negative result.
Oxidase
Urease Test
Test to identify bacteria capable of hydrolyzing
urea using the enzyme urease. The hydrolysis of
urea forms the weak base, ammonia, as one of its
products. This weak base raises the pH of the
media and the pH indicator, phenol red, turns
from yellow to pink.